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人类血小板特异性抗原Siba与糖蛋白Ibα的分子量多态性相关。

Human platelet-specific antigen, Siba, is associated with the molecular weight polymorphism of glycoprotein Ib alpha.

作者信息

Ishida F, Saji H, Maruya E, Furihata K

机构信息

Second Department of Internal Medicine, Shinshu University School of Medicine, Nagano, Japan.

出版信息

Blood. 1991 Oct 1;78(7):1722-9.

PMID:1912562
Abstract

Platelet-specific antigen Sib(a) has been highly implicated in the pathogenesis of refractoriness to human leukocyte antigen (HLA)-matched platelet transfusions in Japan. We provide evidence that the Sib(a) antigen is located on the glycoprotein (GP) Ib alpha and has a close association with the molecular weight (mol wt) polymorphism of GPIb. In modified antigen-capture ELISA (MACE), anti-Sib(a) antibody reacted only with GPIb/IX held by a murine anti-GPIb/IX monoclonal antibody (MoAb). The reactivity of anti-Sib(a) antibody to Sib(a)-positive (Sib(a+)) platelets was abolished after they were treated with Serratia marcescens protease. Platelets from 50 healthy volunteers were semiquantitatively phenotyped for Sib(a) antigen by MACE and divided into three distinct groups: strongly positive, positive, and negative. They were also analyzed by sodium dodeyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and periodic acid-silver staining for mol wt polymorphism of GPIb, phenotyped as A, B, C, or D. Without exception, Sib(a+) platelets showed larger phenotypes (A or B). Removal of sialic acid from Sib(a+) platelets did not reduce the binding of anti-Sib(a). Finally, anti-Sib(a) antibody specifically immunoprecipitated A and B phenotypes of GPIb from Sib(a+) platelets. Thus, Sib(a) antigen evidently is located in the region of glycocalicin that is present only on the A and B phenotypes of GPIb.

摘要

在日本,血小板特异性抗原Sib(a)与人类白细胞抗原(HLA)匹配的血小板输注难治性的发病机制高度相关。我们提供的证据表明,Sib(a)抗原位于糖蛋白(GP)Ibα上,并且与GPIb的分子量(mol wt)多态性密切相关。在改良抗原捕获ELISA(MACE)中,抗Sib(a)抗体仅与由鼠抗GPIb/IX单克隆抗体(MoAb)捕获的GPIb/IX发生反应。用粘质沙雷氏菌蛋白酶处理Sib(a)阳性(Sib(a+))血小板后,抗Sib(a)抗体与它们的反应性消失。通过MACE对50名健康志愿者的血小板进行Sib(a)抗原的半定量表型分析,并将其分为三个不同的组:强阳性、阳性和阴性。还通过十二烷基硫酸钠-聚丙烯酰胺凝胶电泳(SDS-PAGE)和高碘酸-银染色分析GPIb的分子量多态性,表型为A、B、C或D。无一例外,Sib(a+)血小板表现出更大的表型(A或B)。从Sib(a+)血小板中去除唾液酸并不会降低抗Sib(a)的结合。最后,抗Sib(a)抗体从Sib(a+)血小板中特异性免疫沉淀GPIb的A和B表型。因此,Sib(a)抗原显然位于仅存在于GPIb的A和B表型上的糖甘膦区域。

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